Clock gene Per3 deficiency disrupts circadian alterations of gut microbiota in mice

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Circadian rhythms are present in all organisms.The endogenous circadian clock is an autonomous temporal system that generates a rhythm of approximately 24 h even in the absence of environmental signals.The "core" genes in the circadian clock system of mammals consist of Clock and Bmal1, which generate activators, along with Cry1, Cry2, Per1 and Per2, which generate repressors.As one member of the Per family, Per3 is not the "core" clock gene in the usual sense, but it is also essential for physiological regulation in mammals.Per3 exhibits an obvious circadian pattern in peripheral tissues, which is important for the endogenous timing of specific tissues, but its variants have been linked to circadian preference, mental disorders, and cognitive responses to circadian dysregulation [1].
The intestinal microbiota is a complex microbial ecosystem consisting of many species of microbes that can produce metabolites to influence the health of the host and also can communicate with distal organs and impact the functions of organs.The microbiota is associated with maintaining metabolic homeostasis, processing and digestion of nutrients, and participating in the normal metabolism of lipids, which has a strong connection to the incidence of dysbolism, such as diabetes, obesity and cardiovascular disease [2].It has been shown that the intestinal microbiome participates in the development of mental disorders via the gutbrain axis.Strikingly, the circadian clock was reported to impact microbial homeostasis, and daytime-dependent fluctuations were identified in fecal microbiota.These findings suggested that the gut microbiome shows diurnal rhythmicity in humans and laboratory animals.The metabolites produced by microbiota affect the expression of central and liver clock genes and further regulate lipid metabolism.The diurnal pattern of the microbiome is disrupted due to the mutation of the Clock gene, Bmal1 knockout, and Per1/Per2 double mutation.However, the regulatory roles of noncore clock genes in microbiota rhythms are not well understood.Therefore, we investigated the impacts of Per3 deficiency on alterations in the mouse intestinal microbiome in this study.
Male C57BL/6J mice were purchased from the China National Laboratory Animal Resource Center (Shanghai, China).Male and female Per3 +/-mice were purchased from Nanjing Model Animal Center (Nanjing, China), and homozygous Per3 -/-male mice were obtained by expanding the breeding.Mice were divided into six groups with equal numbers, and mice were killed every 4 h, where the onset of light was called ZT0 and lights-off was called ZT12.All animal experiments were carried out according to the protocols of Ethical Standards and Regulations authorized by Zhejiang University of Technology.First, the circadian rhythm expression of some phyla in the intestinal microbiome was tested by qPCR.Then, the cecal contents' 16S rRNA genes V4 region in wild-type (WT) and Per3 -/-mice of ZT4 and ZT16 group were sequenced with Illumina NovaSeq 6000 (Illumina, San Diego, USA) by GUHE Info Technology Co., Ltd.(Hangzhou, China).The collected raw data underwent analysis primarily using QIIME (v1.9.0) and R packages (v3.2.0).The process of assembling paired-end reads and selecting operational taxonomic units (OTUs) was performed by using Vsearch (v2.4.4).
The mRNA expression of Actinobacteria, α-proteobacteria, βproteobacteria and Firmicutes showed that Per3 deficiency altered the circadian rhythm of gut microbes (Figure 1), in which the changes at ZT4 and ZT16 between WT and Per3 -/-mice were significant.Furthermore, we analyzed changes in the cecal contents caused by Per3 deficiency at these two time points.After distinct clustering, the composition of gut microbes showed a great difference between WT and Per3 -/-mice, as well as between ZT4 and ZT16, using principal component analysis (PCA).Our data showed that the difference between WT and Per3 -/-mice at ZT4 was larger than that at ZT16 (Figure 2A).Both the Shannon index and Simpson index were reduced at ZT16 in WT mice compared to those at ZT4 (Figure 2B,C); however, no change in the Shannon index and Simpson index was observed in Per3 -/-mice across the same time points (Figure 2B,C), showing a possible disruption of circadian rhythm caused by Per3 deficiency.Then, specific changes in the composition at the phylum and genus levels were assayed.Increased relative abundances of the phyla Firmicutes, Deferribacteres, TM7 and Verrucomicrobia were observed at ZT4 in Per3 -/- mice compared to those in WT mice, and a reduced trend was observed for the abundances of Bacteroidetes and Actinobacteria.At ZT16, Bacteroidetes were increased, and Proteobacteria, Verrucomicrobia, Cyanobacteria and Deferribacteres exhibited a downward trend relative to controls (Figure 2D).The Firmicutes/ Bacteroidetes ratio (F/B ratio) is generally recognized as a significant factor in maintaining microbiota homeostasis, and its variation is closely related to obesity, inflammatory bowel disease (IBD), hypertension and other diseases [3].In the present study, we demonstrated that the F/B ratio was significantly elevated at ZT4 compared to that at ZT16 in Per3 -/-mice, but no difference was identified in WT mice (Figure 2E).At the genus level, the relative abundances of Ruminococcus, Dorea, and Allobaculum were significantly altered (Figure 2F-H), which is partly consistent with observations in socially isolated mice [4].The relative abundance of Ruminococcus showed a similar change trend to that of the F/B ratio, which is positively associated with the inflammatory response in IBD [5].Additionally, Ruminococcus is associated with tryptamine metabolism, and its metabolites may influence the risk of developing neurological disorders.Lukić et al. [6] demonstrated that antidepressants reduced the abundance of Ruminococcus.The abundance of Dorea was significantly reduced in Per3 -/-mice at ZT4 compared to that in WT mice, which tended to show a negative correlation with the severity of depressive symptoms.Together, our findings confirmed to some extent the roles of Per3 in seasonal mood disorders in a previous report [7].Moreover, the abundance of Allobaculum, which is known as an immunostimulatory species in gnotobiotic mice, was reduced in Per3 -/-mice at ZT16 relative to that at ZT4 and in WT mice.A similar trend was observed in depressive mice, which exhibited a direct relationship with acetic acid and 5-HT [8].In combination with the observations on Dorea and Allobaculum, our findings demonstrate that the altered composition of the gut microbiota caused by Per3 deficiency may be linked to the risk of mood disorders.These observations implied that Per3 deficiency may be associated with inflammation and mood disorders in rodents, which was supported by a previous report [7].Additionally, KEGG analysis showed that Per3 deficiency distinctively leads to alterations in nicotinate and nicotinamide metabolism, lipid biosynthesis proteins, indole alkaloid biosynthesis, energy metabolism and other pathways in mice (Figure 2I).It is noteworthy that Per3 deficiency may affect inflammation, lipid synthesis and mitochondrial homeostasis through the dysregulation of the intestinal microbiome and its circadian rhythm.
Internal circadian rhythms play an essential role in the function of different bodily organs to align environmental signals to achieve maximum efficiency.Recent evidence suggested that the gut microbiome has rhythmicity and exhibits diurnal variations.The biological rhythms of the gut microbiome depend on specific environmental cues within the gut, which fluctuate following dietary intake, host circadian rhythms, behaviors, and other various factors, such as melatonin and body temperature.What is becoming Per3 deficiency disrupts circadian alterations 2005 clear is that not all gut microbiota show diurnal oscillations in their abundance, in which small percentages are called microbial oscillators.These findings support our observations of gut microbiota changes in Per3 -/-mice.Additionally, mutations in circadian clock-related genes have been identified as leading causes of gut microbiota rhythmicity disruption.However, the effect of Per3 on the intestinal microbiome remains unclear.
Our findings demonstrate that Per3 deficiency is related to the disorder of the intestinal microbiota composition and alterations in the rhythm system of the microbiome, particularly at ZT4.Similar phenomena were observed in the core clock gene deficiency mice, including Per1, Per2 and Bmal1, suggesting that the compositions of gut microbes can be altered under conditions of clock gene deficiency in mice.There is extensive evidence suggesting that disruptions in the rhythm of the intestinal microbiome have a strong correlation with metabolic dysfunction, for example, the altered levels of secondary bile acids caused by disrupted rhythm of the microbiome in Bmal1-deficient mice, which was similar to those discovered in patients with type 2 diabetes and obesity [9].These disruptions were also reported to be correlated with the development of neurological conditions.Sun et al. [10] revealed that cognitive impairment in mice can be alleviated by restoring the damaged intestinal microbiome with Dendrobium officinale polysaccharide.Mutations in the Clock gene lead to elevated anxietylike behaviors in mice, which might be associated with disruptions in the circadian rhythm of the microbiome.
In conclusion, our results provide insights into the functional consequences of Per3 on the disruption of the gut microbiome composition and may aid in improving our understanding of how the human gut microbiota is regulated by the circadian clock.